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THE  ELECTRON  MICROSCOPE
Introduction
Introduction
Introduction
Introduction
Introduction
Introduction
Introduction
Introduction
Introduction
Introduction
[object Object],[object Object]
Electron Microscope ,[object Object],[object Object],The two types are:  Scanning and Transmission
Which is the most powerful kind of microscope?
THE LIGHT MICROSCOPE v THE ELECTRON MICROSCOPE   fluorescent (TV) screen, photographic film Human eye (retina), photographic film Focussing screen Vacuum Air-filled Interior Magnets Glass Lenses High voltage (50kV) tungsten lamp Tungsten or quartz halogen lamp Radiation source x500 000 x1000 – x1500 Maximum magnification 0.2nm Fine detail app. 200nm Maximum resolving power Electrons app. 4nm Monochrome Visible light 760nm (red) – 390nm  Colours visible Electromagnetic spectrum used ELECTRON MICROSCOPE LIGHT MICROSCOPE FEATURE
THE LIGHT MICROSCOPE v  THE ELECTRON MICROSCOPE Copper grid Glass slide Support Heavy metals Water soluble dyes Stains Microtome only. Slices    50nm Parts of cells visible Hand or microtome slices    20 000nm Whole cells visible Sectioning Resin Wax Embedding OsO 4  or KMnO 4 Alcohol Fixation Tissues must be dehydrated =  dead Temporary mounts  living or dead Preparation of specimens ELECTRON MICROSCOPE LIGHT MICROSCOPE FEATURE
Properties of electron ,[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object]
Electron beam (A) Transmitted electron (B) Inelastically scattered electrons (C) Elastically scattered electrons (D) Back-scattered electrons (E) Secondary electrons X-rays Visible light
[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object]
Working   &  Image formation ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object]
Magnification ,[object Object],[object Object],[object Object],[object Object],[object Object]
Resolution ,[object Object],[object Object],[object Object],[object Object]
Transmission Electron Microscope (TEM) ,[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object]
Basic Systems Making Up a Transmission Electron Microscope ,[object Object],[object Object],[object Object]
Basic Systems Making Up a Transmission Electron Microscope ,[object Object],[object Object]
Page 167 TABLE 6.3 Major Column Components of the TEM* Component Synonyms Function of Components Illumination System Electron Gun Gun, Source Generates electrons and provides first coherent crossover of electron beam Condenser Lens 1 C1, Spot Size Determines smallest illumination spot size on specimen (see Spot Size in Table 6.4) Condenser Lens 2 C2, Brightness Varies amount of illumination on specimen — in combination with C1 (see Brightness in Table 6.4) Condenser Aperture C2 Aperture Reduces spherical aberration, helps control amount of illumination striking specimen
Specimen Manipulation System Specimen Exchanger Specimen Air Lock Chamber and mechanism for inserting specimen holder Specimen Stage Stage Mechanism for moving specimen inside column of microscope Imaging System Objective Lens — Forms, magnifies, and focuses first image (see Focus in Table 6.4) Objective Aperture — Controls contrast and spherical aberration Intermediate Lens Diffraction Lens Normally used to help magnify image from objective lens and to focus diffraction pattern Intermediate Aperture Diffraction Aperture, Field Limiting Aperture Selects area to be diffracted Projector Lens 1 P1 Helps magnify image, possibly used in some diffraction work Projector Lens 2 P2 Same as P1
Observation and Camera Systems Viewing Chamber — Contains viewing screen for final image Binocular Microscope Focusing Scope Magnifies image on viewing screen for accurate focusing Camera — Contains film for recording
Scanning Electron Microscopy (SEM) Visualizes  Surface  Features
[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object]
Layout and performance of SEM 1-3 Electron gun 4, 10 Aperture 5-6 Condenser lenses 7 Scanning coils 8 Stigmator 9 Objective lens 11 X-ray detector 12 Pre-amplifier 13 Scanning circuits 14 Specimen 15 Secondary electron detector 16-18 Display/Control circuits
Specimen Preparation Specimens are coated with metals to deflect electrons from a beam scanned across the sample.
SEM  of Stereocilia Projecting from a Cochlear (inner ear) Hair Cell
Copper grid slides © 2007 Paul Billiet  ODWS
Higher Resolution Is Achieved by Viewing Sections of Fixed, Stained, and Embedded Samples A microtome cutting sections of an embedded sample.
Microtome knife © 2007 Paul Billiet  ODWS
Fig. 3-22

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Electron microscope

  • 1. THE ELECTRON MICROSCOPE
  • 12.
  • 13.
  • 14. Which is the most powerful kind of microscope?
  • 15. THE LIGHT MICROSCOPE v THE ELECTRON MICROSCOPE fluorescent (TV) screen, photographic film Human eye (retina), photographic film Focussing screen Vacuum Air-filled Interior Magnets Glass Lenses High voltage (50kV) tungsten lamp Tungsten or quartz halogen lamp Radiation source x500 000 x1000 – x1500 Maximum magnification 0.2nm Fine detail app. 200nm Maximum resolving power Electrons app. 4nm Monochrome Visible light 760nm (red) – 390nm Colours visible Electromagnetic spectrum used ELECTRON MICROSCOPE LIGHT MICROSCOPE FEATURE
  • 16. THE LIGHT MICROSCOPE v THE ELECTRON MICROSCOPE Copper grid Glass slide Support Heavy metals Water soluble dyes Stains Microtome only. Slices  50nm Parts of cells visible Hand or microtome slices  20 000nm Whole cells visible Sectioning Resin Wax Embedding OsO 4 or KMnO 4 Alcohol Fixation Tissues must be dehydrated = dead Temporary mounts living or dead Preparation of specimens ELECTRON MICROSCOPE LIGHT MICROSCOPE FEATURE
  • 17.
  • 18.
  • 19. Electron beam (A) Transmitted electron (B) Inelastically scattered electrons (C) Elastically scattered electrons (D) Back-scattered electrons (E) Secondary electrons X-rays Visible light
  • 20.
  • 21.
  • 22.
  • 23.
  • 24.
  • 25.
  • 26.
  • 27.
  • 28.
  • 29.
  • 30.
  • 31.
  • 32.
  • 33.
  • 34. Page 167 TABLE 6.3 Major Column Components of the TEM* Component Synonyms Function of Components Illumination System Electron Gun Gun, Source Generates electrons and provides first coherent crossover of electron beam Condenser Lens 1 C1, Spot Size Determines smallest illumination spot size on specimen (see Spot Size in Table 6.4) Condenser Lens 2 C2, Brightness Varies amount of illumination on specimen — in combination with C1 (see Brightness in Table 6.4) Condenser Aperture C2 Aperture Reduces spherical aberration, helps control amount of illumination striking specimen
  • 35. Specimen Manipulation System Specimen Exchanger Specimen Air Lock Chamber and mechanism for inserting specimen holder Specimen Stage Stage Mechanism for moving specimen inside column of microscope Imaging System Objective Lens — Forms, magnifies, and focuses first image (see Focus in Table 6.4) Objective Aperture — Controls contrast and spherical aberration Intermediate Lens Diffraction Lens Normally used to help magnify image from objective lens and to focus diffraction pattern Intermediate Aperture Diffraction Aperture, Field Limiting Aperture Selects area to be diffracted Projector Lens 1 P1 Helps magnify image, possibly used in some diffraction work Projector Lens 2 P2 Same as P1
  • 36. Observation and Camera Systems Viewing Chamber — Contains viewing screen for final image Binocular Microscope Focusing Scope Magnifies image on viewing screen for accurate focusing Camera — Contains film for recording
  • 37. Scanning Electron Microscopy (SEM) Visualizes Surface Features
  • 38.
  • 39.
  • 40.
  • 41. Layout and performance of SEM 1-3 Electron gun 4, 10 Aperture 5-6 Condenser lenses 7 Scanning coils 8 Stigmator 9 Objective lens 11 X-ray detector 12 Pre-amplifier 13 Scanning circuits 14 Specimen 15 Secondary electron detector 16-18 Display/Control circuits
  • 42. Specimen Preparation Specimens are coated with metals to deflect electrons from a beam scanned across the sample.
  • 43. SEM of Stereocilia Projecting from a Cochlear (inner ear) Hair Cell
  • 44. Copper grid slides © 2007 Paul Billiet ODWS
  • 45. Higher Resolution Is Achieved by Viewing Sections of Fixed, Stained, and Embedded Samples A microtome cutting sections of an embedded sample.
  • 46. Microtome knife © 2007 Paul Billiet ODWS

Editor's Notes

  1. © Ryan Barrow 2008